Abstract

As breast volume may be associated with heart cancer risk, we studied the relationship between breast volume, CYP1A2*1F and coffee intake. Among healthy premenopausal non-hormone users, 3+ cups per day was associated with lower volume only in C-allele carriers (Pinteraction=0.02), which is consistent with reports that coffee protects only C-allele carriers against breast cancer.

Mammographic density is a strong risk factor for breast cancer (Boyd et al, 2005), the risk increasing with larger percentage density. The non-inducible CYP1A2*1F C-allele was associated with the percent density in normal-weight postmenopausal women not using hormone therapy (Takata et al, 2007). CYP1A2 enzyme activity has also been associated with density (Hong et al, 2004), and coffee induces CYP1A2 enzyme activity (Djordjevic et al, 2007). There is no direct correlation between breast density and size after adjustment for waist-to-hip ratio and BMI (Beijerinck et al, 1995). However, a larger breast size has been associated with increased breast cancer risk (Kato et al, 1995), especially in lean women (Kusano et al, 2006) or in women with proliferative breast disease (Dupont and Page, 1987). We therefore investigated whether coffee intake was associated with breast volume in young women and whether any association was modified by the CYP1A2*1F genotype.

Materials and methods

A total of 269 young healthy Swedish women from breast cancer high-risk families volunteered to participate in this study between 1996 and 2006. The study population has previously been described in detail (Hietala et al, 2008). The Ethics Committee of Lund University approved the study. All women signed a written informed consent.

The questionnaire included questions on reproductive factors, the use of hormonal contraceptives, smoking, coffee consumption and so on. One large cup (approximately 300ml) was counted as two traditional cups of coffee (approximately 150ml). Blood samples and body measurements were collected both during menstrual cycle days 5–10 and days 18–23. Breast volumes were measured while the woman was on her hands and knees with the breasts hanging down. The volume was approximated to a pyramid (base area × height/3). Total breast volume, that is the sum of the right and left breast volumes, was calculated in each visit.

Mutation testing of the BRCA1 and BRCA2 genes was not performed as part of this study and carrier status was obtained from the clinical records as previously described (Hietala et al, 2008). CYP1A2*1F analysis (rs762551) PCR primers 5′-AGGTATCAGCAGAAAGCCAGCAC and 5′-GCTGAGGGTTGAGATGGAGACAT were used as described earlier (Bågeman et al, 2008). Thirty-eight samples were run in duplicate with 100% concordance.

Oestradiol was analysed with Elecsys system 1010/2010 in EDTA plasma. This system uses a competitive immunoassay with a polyclonal antibody directed towards 17-β oestradiol. Intra-assay variation ranged from 1.9 to 5.7% and the inter-assay variation varied from 2.3 to 6.2%.

The statistical software programs SPSS13.0 and STATA 10.0 were used. Breast volumes and weights were not normally distributed and were transformed using the natural logarithm (ln). The CYP1A2*1F genotype was classified into two groups (A/A or any C-allele). An interaction term was calculated between CYP1A2*1F and coffee (3+ cups per day). Multivariate linear regression analyses were performed to evaluate the interaction between CYP1A2*1F and coffee on breast volume, and further adjusted for family clustering using the cluster option of the logistic command in STATA. Geometric means of standardised breast volumes and 95% prediction intervals were calculated. The breast volumes were standardised at age 29 years, weight (ln67kg), non-smoking and nulliparity. Multivariate logistic regression was used to analyse the association between coffee and hormone and growth factor levels. A P-value of <0.05 was taken to be significant. All P-values were two sided.

Results

Characteristics of the 269 women and CYP1A2*1F genotypes are presented in Table 1. CYP1A2*1F were available for 267 of the 269 women. CYP1A2*1F did not differ according to BRCA1/2 mutation status (Table 2). Coffee consumption did not significantly differ between the CYP1A2*1F after adjusting for age and smoking.

BRCA1/2 mutation status and CYP1A2*1F genotypes in the women included in the study. CYP1A2*1F genotypes were missing for two women from non-BRCA1/2 families

Total breast volumes during menstrual cycle days 18–23 were available for 255 women who were not currently breast-feeding and without previous breast surgeries. Age-adjusted coffee consumption was positively associated with current smoking (P<0.0001), but not with nulliparity or current hormonal contraception. Total breast volumes were positively associated with weight (β=2.119; P<0.0001), but not with age, current hormonal contraception, nulliparity, current smoking or CYP1A2*1F.

Among the non-users, of whom 145 had available breast volumes and CYP1A2*1F genotypes, the association between a moderate-to-high coffee consumption (3+ cups per day) and breast volume was significantly modified by CYP1A2*1F genotype. Among women carrying at least one C-allele, moderate-to-high consumption was associated with lower standardised breast volumes compared with low consumption (896 vs 749ml) whereas the standardised volumes were somewhat larger in women with moderate-to-high coffee consumption and the A/A genotype (797 vs 847ml) (β=−0.303; Pinteraction=0.02) (Figure 1). The interaction remained significant after further adjustment for BRCA1/2 mutation status (β=−0.304; P=0.02) and after exclusion of women who currently smoked or used snuff (β=−0.328; P=0.03). The women belonged to 105 different families. The interaction remained significant after adjustment for family clustering (P=0.03).

The figure shows the geometric means of the breast volumes in women according to their CYP1A2*1F genotype and coffee consumption. The breast volumes were standardised at age 29 years, body weight ln67kg, nulliparity and non-smoking....

Plasma concentrations of oestradiol, progesterone, testosterone, SHBG, IGF-1 and IGFBP-3, obtained during the visit when the breast volumes were measured, were available for 139 women with data on breast volumes and CYP1A2*1F. In this subgroup, the interaction between coffee consumption and CYP1A2*1F genotype on breast volume was somewhat stronger (β=−0.341; Pinteraction=0.007) and became even stronger after further adjustment for hormone and growth factor levels (β=−0.401; Pinteraction=0.002).

Among current hormonal contraceptive users, coffee consumption was not associated with breast volume and there was no significant interaction between coffee and CYP1A2*1F on breast volume.

Discussion

Our main finding was a significant interaction between coffee consumption, CYP1A2*1F genotype and breast volume among young healthy women who did not use hormonal contraceptives. This interaction was mainly driven by the fact that a moderate-to-high coffee intake was associated with lower breast volume in women with the C-allele. No association between coffee and breast volumes was observed in women with the CYP1A2*1F A/A genotype or in women who currently used hormonal contraception. As hormonal contraceptives lower the CYP1A2 enzyme activity (Rietveld et al, 1984), the latter observation was expected.

In this study, approximately 50% of the women carried the CYP1A2*1F A/A genotype, which is consistent with reported frequencies (Sachse et al, 1999; Nordmark et al, 2002). CYP1A2*1F is located in intron 1 and may not directly be associated with enzyme activity, but is rather linked to other polymorphisms with regulatory properties (Sachse et al, 1999). Coffee has been reported to predict 4% of the variation in CYP1A2 enzyme activity (Le Marchand et al, 1997).

In this study, breast volume was measured and approximated to a pyramid for practical reasons. A more exact procedure may have been to use water displacement, which we tried, but was impractical and less reproducible. Using bra cup size as a measurement of breast volume is less satisfactory, as cup-size labelling is not standardised (Ringberg et al, 2006).

Neither bra cup size nor breast volume reflects how much of the women's breast volume consists of breast parenchyma and how much is fat. A high BMI is positively correlated with larger cup sizes (Hall et al, 1999), which is in line with our findings. Others have reported that larger breasts consist of proportionally more fat and less parenchyma than smaller breasts in premenopausal women (Beijerinck et al, 1995; Kato et al, 1995). Most of our women were too young to have undergone mammography. We were thus unable to address whether coffee was associated with density, which is a stronger predictor of breast cancer risk than breast volume.

As coffee consumption was associated with lower breast volume among carriers of the C-allele with little effect among homozygous A/A carriers, mechanisms other than the induction of the CYP1A2 enzyme may be at play. Caffeine is the only major compound in coffee that is known to be metabolised by CYP1A2 and the effect could be attributed to the prolonged exposure of caffeine among C-allele carriers, as caffeine inhibits cell proliferation in mouse epidermal JB6 cells (Hashimoto et al, 2004).

Intake of caffeine has been positively associated with SHBG levels (Nagata et al, 1998) and inversely associated with bioavailable testosterone (Ferrini and Barrett-Connor, 1996), but CYP1A2*1F was not analysed. In this study, we did not observe any significant associations between coffee intake and hormone and growth factor levels. However, bioavailable testosterone levels were positively associated with breast volumes in both groups (data not shown). In contrast to our earlier study, we did not find that hormonal contraception significantly influenced breast volume (Jernström and Olsson, 1997). In this study, measured hormone levels did not explain the observed interaction between coffee and CYP1A2*1F on breast volume, although this became stronger after further adjustment for hormone levels.

In conclusion, the CYP1A2*1F genotype significantly modified the relationship between coffee consumption and breast volume in non-users of hormonal contraception. It is likely that various compounds in coffee exert a direct effect on the breast epithelium. As breast volume is associated with breast cancer risk in lean women, our finding is compatible with earlier reports of a protective effect of coffee on breast cancer risk restricted to women with the CYP1A2*1F C-allele.

Acknowledgments

This study was supported by grants from Vetenskapsrådet, (The Swedish Research Council, K2001-27GX-14120-01A and K2008-68X-20802-01-3), the Medical Faculty in Lund, the Mrs. Berta Kamprad's Foundation, The Gunnar Nilsson Foundation, The South Swedish Health Care Region (Region Skåne), Lund Hospital Fund and the Swedish Cancer Society. We thank our research nurses Kerstin Nilsson, Monica Pehrsson, Karin Henriksson and Anita Schmidt-Casslén for their assistance with body measurements and blood drawing, and Johanna Wagenius, Johanna Frenander, Helen Sundberg, Malin Sternby and Susanna Holmquist for their assistance with recruitment. Dr Åke Borg was responsible for BRCA1 and BRCA2 mutation testing. We thank Dr Pär-Ola Bendahl, biostatistician, for assistance with calculation of the prediction intervals and family-clustering models. We thank Dr Eric T Dryver for proofreading the manuscript.